Metabolic thermotolerance: magnetic resonance detected protection of

Aug 30, 1991 - Glutamate Synthase1-. T. M. Logan, P. Zhong, and D. G. Lynn*. *. Department of Chemistry, University of Chicago, 5735 Ellis Avenue, Chi...
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Biochemistry 1992, 31, 7256-7263

7256

Metabolic Thermotolerance: Magnetic Resonance Detected Protection of Glutamate Synt haset T. M. Logan, P. Zhong, and D. G. Lynn' Department of Chemistry, University of Chicago, 5735 Ellis Avenue, Chicago, Illinois 60637 Received August 30, 1991; Revised Manuscript Received March 19, I992

Metabolism in maize meristem cultures exposed to different heat treatments has been analyzed by W - N M R spectroscopy of tissue extracts. The effects of a 40 OC permissive stress were compared with a 45 O C lethal stress, and the metabolism of glutamate and glutamine were markedly altered by both temperatures. Changes in the incorporation of labeled precursors, alterations due to the in vivo application of enzyme inhibitors, and differences in the activity of enzymes in cell free extracts have confirmed that glutamate synthase (GluS) is partially inactivated by the lethal thermal exposure. This enzyme is quantitatively protected by the induction of thermotolerance. The time dependence for the protection correlates with the appearance of a set of late-arising heat shock proteins (hsps). The function of these late-arising proteins is not yet known, but only one of them, a 67-kDa protein, is spatially correlated with GluS protection. Therefore, the quantitative protection of a key metabolic enzyme has been correlated with the in vivo function of a specific hsp. ABSTRACT:

Organisms must orchestrate an intricate and highly interdependent series of metabolic reactions to ensure viability. In any such network or series the weakest step defines the limits on the viability of the entire network. In the evolution of a metabolic network, a more durable enzyme catalyst may be in the process of forming or inherent physical limitations on the chemical transformation itself may have forced a separate protective mechanism to have developed. The transcriptionally controlled stress responses appear to represent such a separate protective strategy. The universal biological response to elevated temperatures is the rapid synthesis of a set of so-called heat shock proteins, or hsps' (Lindquist, 1986; Lindquist & Craig, 1988; Vierling, 1991). While there is considerable variability in the number and molecular weight distributions and in the temperature required for inducing hsp synthesisamong different organisms, the hsps are among the most highly conserved proteins in nature and undoubtedlyserve common criticalfunctions (Craig & Gross, 1991; Pechan, 1991; Gething & Sambrook, 1992). While the heat shock response has been intensely studied for the last decade, still little is known regarding the specific chemical and biochemical functions of these proteins. A link between the presence of abnormal or denatured proteins and hsp synthesishas been established. Osmotic shock (Bonham-Smith et al., 1987), ethanol, abscissic acid (Heikkila, 1984), amino acid analogues and puromycin treatments (Hightower, 1980; Goff & Goldberg, 1985), and even the injection of denatured proteins (Anathan et al., 1986) elicit some subset of hsp synthesis. In vitro, these hsps bind to denatured protein aggregates (Pelham, 1986; Palleros et al., 1991), bind to nascent polypeptide chains on the ribosome (Lindquist & Craig, 1988; Rothman, 1989), facilitate translocation of proteins across membranes (Deshaies et al., 1988; Chirico et al., 1988),refold and assemble translocated proteins (Hemmingsen et al., 1988; Prasad & Hallberg, 1989; Ellis, This work was supported by the CIBA-GEIGY Corporation, The Midwest Plant Biotechnology Consortium, and Dow Chemical Co. * To whom correspondence should be addressed. I Abbreviations: GluS, glutamate synthase; GDH, glutamate dehydrogenase; GS, glutamine synthetase; hsp, heat shock protein; Glu-y, glutamate C-4; Gln-7, glutamine C-4; gdw, gram dry weight.

1990), and bind to and stabilize organellar membranes (Ignolia h Craig, 1982; Vierling, 1991). The hsps, then, are induced by denatured proteins and interact with denaturing protein domains. The proteinswhich require such stabilization in vivo during such heat shocks are, however, unknown. Leenders et al. (1974) demonstrated a link between respiratory metabolism and the heat shock response of Drosophila. Application of respiratory inhibitors such as azide, salicylate, or rotenone or anaerobic conditions resulted in a stimulation of the samechromosomal regions as did heat shock. Chou et al. (1989) have shown that thermotolerated soybeans contained a higher fraction of mitochondria which remained coupled at elevated temperatures in in vitro oxygen consumption assays. Localization of hsps to the chloroplast (Amir-Shapira et al., 1990; Marshall et al., 1990; Vierling et al., 1986) or to the mitochondria (Nieto-Sotelo, et al., 1990) may function to protect specific metabolic reactions compartmentalized to those organelles. In addition, principle metabolic enzymes including enolase (Iida & Yahara, 1985), phosphoglycerate kinase, and GAPDH (Piper et al., 1988) have been shown to be heat shock proteins. Therefore, it appears that the heat shock response has evolved to protect biological reactions, including the reactions of primary metabolism, against thermal stress. The question as to which reactions require such protection remains. This report details the use of W N M R methods (London, 1988; Cohen, 1989) to assign one of these metabolic weak links in maize meristem cultures to glutamate synthase (GluS), the primary enzyme of glutamate/glutamine metabolism.

METHODS AND MATERIALS Tissue Culturing and Sampling Preparation. Maize seeds (Zea mays, var MX085A flats; OLDS Seed Co., Madison WI 53707) were surface sterilizedby immersion in 1:1 bleach: HzO for 20 min. The seeds were exhaustively rinsed with 10 volumes of sterilized water and hydrated for 4 h at room temperature. The seeds were planted on moistened sterile trays, wrapped in foil, and germinated at ambient temperature (25 f 1 "C). After three days, the terminal 5-7 mm of the root tip was removed and approximately 150 root tips were placed

0006-2960/92/0431-7256$03.00/0 0 1992 American Chemical Society

Metabolic Thermotolerance in sterile 125-mL Erlenmeyer flasks containing 7 mL of White's medium (White, 1943)with 1mM NaOAcas a carbon source. The cultures were shaken (70 rpm) in the dark for 24 h before an additional milliliter of medium was added which contained sufficient sodium acetate, either at natural abundance or 99% [2J3C]acetate, to give a final 10 mM acetate concentration. The cultures were maintained under these conditions for 45 min at the indicated temperatures. Following excision, plant tissues mount a wound response which includes altered respiration and increased metabolic fluxes through specificpathways (Uritani & Asahi, 1980). Culturing the roots for 24 h prior to metabolite analysis allowed sufficient time for the wound response to maximize and decline. Application of Temperature Stresses. The cultured corn root tips were exposed to either 40 OC or 45 OC heat shock for 45 min coincidentwith the acetate feeding in a temperaturecontrolled ( f l "C) shaken water bath. The culturing roots were covered with foil during the heat shocks to maintain etiolated conditions. Following the methods of Lin et al. (1984), thermotolerance was induced by exposing the root tip cultures to a 10-min, 45 O C stress in the water bath shaker followed by an immediate return to 24 OC. These cultures were maintained for up to 4 h before the additional 1 mL of media was added to give the final 10mM acetate concentration and they were exposed to the desired temperature treatment for 45 min. Tissue Extraction and N M R Sample Preparation. I3CNMR samples were collected from a minimum of six replicate flasks, corresponding to about 1000 separate meristematic tips. The root tissues were collected with a minimum of handling (Wallace et al., 1984), rinsed with HzO, and quickly frozen with liquid N2. The frozen roots were lyophilized to dryness and combined into two separate samples, and the dry weights were obtained. The dried samples, ranging from 150 to 300 mg, were ground to a fine powder with a mortar and pestle and extracted overnight at 4 OC with 5% HC104 (approximately 10 mL). Insoluble material was removed by vacuum filtration through Whatmann No. 1 filter paper, and the filtrate was neutralized to pH 7.0 with 3 N KOH. The precipitate that formed during the neutralization was removed by vacuum filtration, and the filtrate was lyophilizedto dryness. The lyophilized powder was suspended in a minimum of cold H20 (